Classifications

• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
  • G01N21/17—Systems in which incident light is modified in accordance with the properties of the material investigated
  • G01N21/55—Specular reflectivity
  • G01N21/552—Attenuated total reflection
  • G01N21/553—Attenuated total reflection and using surface plasmons
  • G01N21/554—Attenuated total reflection and using surface plasmons detecting the surface plasmon resonance of nanostructured metals, e.g. localised surface plasmon resonance
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
  • G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
  • G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
  • G01N33/53—Immunoassay; Biospecific binding assay; Materials therefor
  • G01N33/543—Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals
  • G01N33/54313—Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals the carrier being characterised by its particulate form
  • G01N33/54346—Nanoparticles
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
  • G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
  • G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
  • G01N33/53—Immunoassay; Biospecific binding assay; Materials therefor
  • G01N33/543—Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals
  • G01N33/551—Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals the carrier being inorganic
  • G01N33/553—Metal or metal coated
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
  • G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
  • G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
  • G01N33/53—Immunoassay; Biospecific binding assay; Materials therefor
  • G01N33/558—Immunoassay; Biospecific binding assay; Materials therefor using diffusion or migration of antigen or antibody
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N2469/00—Immunoassays for the detection of microorganisms
  • G01N2469/10—Detection of antigens from microorganism in sample from host
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N2469/00—Immunoassays for the detection of microorganisms
  • G01N2469/20—Detection of antibodies in sample from host which are directed against antigens from microorganisms

Definitions

• the present invention relates to systems and methods for detecting target analytes in a sample.
• the present invention provides a localized surface plasmon resonance- based analyte detection system capable of detecting a minute quantity of a target analyte in a sample.
• LSPR local surface plasmon resonance
• the present application describes the use of localized surface plasmon resonance (LSPR) techniques for performing assays involving specific binding partners including, but not limited to, ligands, receptors, transcription factors, binding DNA elements, antigens, and antibodies. More specifically, the present application relates to processes and materials for achieving significant amplification in such assays using nanostructure-binding partner conjugates. In some aspects, the present disclosure provides compositions and methods for achieving sensitive detection of molecules using LSPR techniques, and minimizing non-specific binding (NSB) levels in the assays provided.
• NBS non-specific binding
• the present application relates to nanostructure- binding partner conjugates, wherein the nanostructures are metallic nanostructures comprising a plurality of spikes.
• the nanostructures are metallic nanostructures having an average diameter of at least 50 nm.
• the nanostructures are metallic nanostructures having an average diameter of about 50 nm to about 120 nm.
• the present disclosure provides the use of such metallic nanostructure-binding partner conjugates in solution to determine the binding of specific binding partners in a qualitative or quantitative manner.
• the present disclosure provides methods for generating the conjugates described herein.
• the present disclosure provides methods and compositions for detecting a target analyte in a sample, the method comprising mixing the sample with a first detection conjugate and a second detection conjugate in a solution, wherein the first and second detection conjugates comprise nanostructures coupled to binding partners that are capable of specifically binding to the target analyte if present in the sample to form a complex between the first detection conjugate, the analyte, and the second detection conjugate.
• the nanostructures are anisotropic nanostructures that comprise a plurality of protrusions on spherical cores and wherein the average tip to tip diameter of the nanostructures is at least about 50nm.
• the average diameter of the nanostructures is about 70 nm or about 90 nm.
• the nanostructures are spherical nanostructures.
• the methods further comprise exposing the complex to a light source at a wavelength range within the ultraviolet-visible-infrared spectrum.
• the methods comprise measuring an optical signal from the complex, wherein a change in the optical signal indicates the presence of the target analyte in the sample.
• more than two detection conjugates are used. For example, a third, a fourth, a fifth, or more detection conjugates are added.
• each of the detection conjugates is capable of binding to the same target analyte to form a complex.
• each of the detection conjugates binds to non-overlapping epitope(s) on the target analyte.
• some or all of the conjugates are anisotropic.
• the mixing step occurs in the presence of 3-((3-Cholamidopropyl) dimethylammino)-l-propanesulfonate (CHAPS).
• CHAPS 3-((3-Cholamidopropyl) dimethylammino)-l-propanesulfonate
• the CHAPS is present at a concentration of about 0.1% w/v to about 0.5% w/v. In further embodiments, the CHAPS is present at a concentration of about 0.2% w/v.
• the solutions provided herein comprise CHAPS.
• the mixing step occurs in the presence of a polymeric material selected from polyethylene glycol (PEG), polyvinylpyrrolidone, methylcellulose, dextrans, poiyailylamme, polyethyleneimine, poiylysine, polyacrylic acid, polyglutamic acid, polyvinylalcohol, and polyaspartic acid.
• a polymeric material selected from polyethylene glycol (PEG), polyvinylpyrrolidone, methylcellulose, dextrans, poiyailylamme, polyethyleneimine, poiylysine, polyacrylic acid, polyglutamic acid, polyvinylalcohol, and polyaspartic acid.
• the polymeric material is PEG.
• PEG is present at a concentration from about 0.05% to about 5% w/v, or from about 0.1% to about 3%.
• the PEG has a molecular weight of 1,000 to 300,000, or 2,000 to 250,000, or 3,000 to 200,000.
• the mixing step occurs in the presence of a viscosity enhancer.
• the solutions provided herein comprise a viscosity enhancer.
• the viscosity enhancer selected from trehalose, maltodextrin, sucrose, sorbitol, mannitol, polyvinylpyrrolidone (PVP), polyvinyl alcohol (PVA), cyclodextrins, randomly alkylated cyclodextrins, methylcellulose, trehalose, sucrose, sorbitol, mannitol and ficoll, dextran, or any combination thereof.
• the mixing step occurs in the presence of dextran at a concentration from about 0.05% to about 5%, depending on the molecular weight.
• dextran is present at a concentration of about 0.05%, about 0.1%, about 0.5%, about 1%, about 1.5%, about 2%, about 2.5%, about 3%, about 3.5%, about 4%, about 4.5%, or about 5%. .
• the mixing step occurs in the presence of gelatin.
• the solutions provided herein comprise gelatin.
• the gelatin is present at a concentration of between about 0.1% to about 3%,
• solutions and reaction mixtures provided herein comprise at least one binding partner-nanostructure conjugate, CHAPS buffer, PEG, one or more Hofmeister series salts, EDTA, a polymer-based blocking reagent such as a Biolipidure®, BSA, gelatin, or any combination thereof.
• the Hofmeister series salt is magnesium chloride.
• the Hofmeister series salt is calcium chloride.
• the reaction mixture comprises multiple salts such as Hofmeister series salts.
• the solutions and reaction mixtures provided herein comprise MgCL2 or NaSCN at a concentration of about lOmM to about 250mM, or at a concentration of about lOOmM.
• the solutions and reaction mixtures provided herein comprise a citrate of the bivalent cation, for example, a citrate of Mg2+ or a citrate of Ca2+.
• the solutions and reaction mixture comprises thiocyanate, manganese, cobalt, nickel, ethylenediaminetetraacetic acid (EDTA) and/or ethylene glycol-bis(P-aminoethyl ether)- ⁇ , ⁇ , ⁇ ', ⁇ '-tetraacetic acid (EGTA)).
• the EDTA and/or EGTA is present in the solution at a concentration of about 5mM to about lOOmM.
• the nanostructures employed in the methods and compositions provided herein comprise a plurality of protrusions, wherein the average tip-to-tip diameter of the nanostructures is about 50 nm, about 60 nm, about 70 nm, about 80 nm, about 90 nm, about 100 nm, about 110 nm, or about 120 nm.
• the nanostructures are metallic nanostructures.
• the nanostructures are gold metallic nanostructures.
• the nanostructures provided herein are spherical nanostructures.
• the average diameter of the spherical nanometers is about 50 nm, about 60 nm, about 70 nm, about 80 nm, about 90 nm, about 100 nm, about 110 nm, or about 120 nm.
• the present disclosure provides methods of detecting a target analyte in a sample comprising: (a) mixing the sample with a first detection conjugate, a second detection conjugate, CHAPS, bovine serum albumin (BSA), one or more polymeric material, one or more viscosity enhancer, a salt, and optionally a chelator, in a solution, wherein the first and second detection conjugates comprise nanostructures coupled to binding partners that are capable of specifically binding to the target analyte if present in the sample to form a complex between the first detection conjugate, the analyte, and the second detection conjugate; (b) exposing the complex to a light source at a wavelength range within the ultraviolet-visible-infrared spectrum; and (c) measuring an optical signal from the complex, wherein a change in the optical signal indicates the presence of the target analyte in the sample.
• the polymeric material is selected from the group consisting of PEG, polyvinyl pyrrolidone, gelatin, methylcellulose, dextran, polyallylamine, poly ethyl eneimine, polylysine, polyacrvlic acid, polyvinylalcohol, and polyaspartic acid.
• the viscosity enhancer is selected from the group consisting of trehalose, maltodextrin, sucrose, sorbitol, mannitol, polyvinylpyrrolidone (PVP) polyvinyl alcohol (PVA), cyclodextrin, methylcellulose, dextran, and ficoll.
• the salt is selected from the group consisting of NaCl, MgC12, CaCh, and NaSCN.
• the chelator is selected from the group consisting of Ethylenediaminetetraacetic acid (EDTA) and ethylene glycol-bis(P-aminoethyl ether)-N,N,N',N'-tetraacetic acid (EGTA).
• the solutions and reaction mixtures provided herein comprise a Biolipidure® reagent.
• the Biolipidure® reagent is Biolipidure® 205, 206, 1002, 1201, 1202, or a combination thereof.
• the nanostructures are selected from the group consisting of spherical nanoparticles and nanoparticles comprising a plurality of protrusions.
• the present disclosure provides methods, solutions, and reaction mixtures comprising a first detection conjugate, a second detection conjugate, CHAPS, BSA, gelatin, PEG, EDTA, MgC12, a Biolipidure® reagent, or any combination thereof.
• the optical signal is reflectance, an absorbance spectrum, scattering spectrum, or an emission spectrum.
• the change in the optical signal comprises a spectral peak wavelength shift and/or a total spectral profile shift.
• the total spectral profile shift is a difference spectrum.
• the methods provided herein provide detection of nanogram, picogram, or femtogram quantities of the target analyte. [0020] In some embodiments, the methods provided herein are performed in a spectrophotometric cuvette, an analytical rotor, a microwell plate, a clinical analyzer, a flow chamber, on the tip of an optical fiber, or in a transparent gel.
• the present disclosure provides a reaction mixture comprising at least one binding partner-nanostructure conjugate, wherein the nanostructures comprise a plurality of protrusions and wherein the average diameter of the nanostructures is at least about 50nm, or at least about 70 nm, or at least about 90 nm, or at least about 120 nm.
• present disclosure provides a reaction mixture comprising at least one binding partner-nanostructure conjugate, wherein the nanostructures are spherical nanostructures.
• the reaction mixture further comprises a zwitterionic detergent.
• the zwitterionic detergent is selected from the group consisting of 3-((3-Cholamidopropyl) dimethylammino)-l- propanesulfonate (CHAPS), and a sulfobetaine detergent.
• CHAPS is present at a concentration of about 0.1% to about 1%. In further embodiments, the CHAPS is present at a concentration of about 0.5%.
• the binding partner is a biological macromolecule.
• the biological macromolecule is selected from an antibody or a fragment thereof, an antigen, a receptor, a ligand, a polynucleotide, an aptamer, a polypeptide, a polysaccharide, a lipopolysaccharide, a glycopeptide, a lipoprotein, or a nucleoprotein.
• the methods and compositions provided herein comprise a first detection conjugate and a second detection conjugate, wherein one of the binding partners of the detection conjugate is an antibody.
• the first and second detection conjugates both comprise binding partners that are antibodies.
• the antibodies conjugated to the first and second conjugates bind to different epitopes on the same target analyte. In some embodiments, the first and second antibodies or first and second conjugates bind to two different non-overlapping epitopes on the target analyte. In other embodiments, the first and second antibodies or first and second conjugates bind to two different antigens. In some embodiments, the two different antigens are two interacting molecules. In some embodiments, the interacting molecules are two macro-molecules, including but not limited to, a receptor and its ligand (e.g., a protein hormone and its binding receptor), a DNA binding transcription factor and another transcription factor and/or DNA, etc.
• a receptor and its ligand e.g., a protein hormone and its binding receptor
• the target analyte is selected from a protein, enzyme, antigen, antibody, peptide, nucleic acid, hormone, glycoprotein, polysaccharide, toxin, virus, virus particle, drug molecule, hapten, and a chemical.
• the target analyte is a pathogenic antigen or antibody to a pathogenic antigen.
• the pathogenic antigen is a viral antigen.
• the viral antigen is from a virus selected from feline leukemia virus, canine parvovirus, foot and mouth virus, influenza virus, hepatitis a virus, hepatitis b, hepatitis c virus, HIV virus, human papilloma virus, Epstein Barr virus, and rabies virus.
• the pathogenic antigen is a bacterial antigen.
• the bacterial antigen is selected from Ehrlichia, Borrelia, Anaplasma, Salmonella, Bacillus, and Rickettsia.
• the bacterial antigen is selected from Ehrlichia canis, Ehrlichia chaffeensis, Ehrlichia ewingii, Borrelia burgdorferi, Anaplasma platys, Anaplasma phagocytophilum, Salmonella enterica, Bacillus anthracis, and Rickettsia rickettsii.
• the pathogenic antigen is a fungal antigen or a parasitic antigen.
• the fungal antigen or parasitic antigen is selected from canine heartworm, Giardia lamblia, plasmodium falciparum, African trypanosomiasis, and Trypanosoma brucei.
• the mixture of the sample with the first and second detection conjugates provided herein is conducted in the presence of a blocking agent.
• the blocking agent is selected from bovine serum albumin (BSA), casein, gelatin, ovalbumin, and gamma-globulins.
• BSA bovine serum albumin
• the blocking agent is BSA present at a concentration of about 1% to about 5% w/v.
• the present disclosure provides methods for preparing a conjugate comprising a binding partner and anisotropic metallic nanostructure suitable for detecting changes in optical signal based on the presence of a target analyte, wherein the anisotropic metallic nanostructure comprises a plurality of protrusions (spikes) and wherein the diameter of the metallic nanostructure is at least about 50 nm.
• the present disclosure provides methods for preparing a conjugate comprising a binding partner and metallic nanostructures suitable for detecting changes in optical signal based on the presence of a target analyte, wherein the metallic nanostructure is a spherical nanostructure.
• the method comprises mixing a solution comprising the metallic nanostructures with a solution comprising the binding partner to form a binding partner-nanostructure conjugate; blocking the conjugate with a blocking reagent provided herein (e.g., BSA and/or gelatin and/or PEG and/or a Biolipidure® reagent), with or without the presence of a viscosity enhancer and/or one or more Hofmeister series salt and/or EDTA and/or EGTA; (c) centrifuging the conjugate; and (d) resuspending the conjugates in a diluent comprising buffer such as phosphate buffered saline (PBS) or Tris buffered saline (TBS) or borate buffer, a blocking agent provided herein (e.g., BSA and/or gelatin and/or PEG), and CHAPS.
• a blocking reagent provided herein
• the binding partner is an antibody.
• the antibody is an antibody containing hydrophobic regions.
• the metallic nanostructures and/or solution comprising the binding partner further comprises a viscosity enhancer.
• the viscosity enhancer is selected from trehalose, maltodextrin, dextran, sucrose, sorbitol, mannitol, polyvinylpyrrolidone (PVP), and polyvinyl alcohol (PVA).
• the viscosity enhancer is dextran.
• the viscosity enhancer is methylcellulose.
• the centrifugation step of the method for preparing a conjugate provided herein comprises centrifugation at about 2000g or more. In further embodiments, the method comprises centrifugation at about 5000g or more. In further embodiments, the method comprises centrifugation at about 10,000g or more. In further embodiments, the method comprises centrifugation at about 50,000g or more. In further embodiments, the method comprises centrifugation at about 75,000g or more. In further embodiments, the method comprises centrifugation at about 100,000g or more.
• the present disclosure provides a lyophilization step following resuspension of the conjugates.
• the lyophilization step comprises dispensing the conjugates in liquid nitrogen, freeze-drying using vacuum and temperature cycles.
• Figure 1 Illustrates the principle of the LSPR immunoassay described herein.
• the metallic nanoparticle comprising a plurality of spikes by itself exhibits an optical spectrum. Slight changes at the surface of the nanoparticle due to first primary binding and subsequent secondary binding cause progressive changes in the characteristics of the light interacting with the nanoparticle-binding partner conjugates. Such changes can be recorded by a suitable spectrometer and provide qualitative as well as quantitative information.
• Figure 2. Shows the titration of an anti-TSH antibody CI into nanostructures comprising a plurality of protrusions to form antibody-nanostructure conjugates.
• Figure 3 Shows the titration of anti-TSH antibody C6 into nanostructures comprising a plurality of protrusions to form antibody-nanostructure conjugates.
• Figure 4 Shows the large scale (100ml nanostructures) titration of antibodies CI and C6 into nanostructures comprising a plurality of protrusions to form CI antibody- or C6 antibody- nanostructure conjugates.
• the inset shows strips striped with Protein A which have been dipped into the conjugate solutions with or without BSA blocking.
• Figure 5 Shows peak shift of unconjugated (573.8 nm) and CI (shift to 585.3 nm) or C6 (shift to 585.9 nm) nanostructures.
• Figure 6 Shows the peak shifts of unconjugated nanostructures, CI antibody- and C6- antibody nanostructures, and CI antibody and C6-antibody nanostructures after BSA blocking.
• Figure 7 Shows lateral flow strips striped with Protein A (0.5 mg/mL), dipped in a solution containing the conjugated nanostructures generated using the absorptive protocol, or the conjugated nanostructures generated using the absorptive protocol and blocked with BSA.
• Figure 8. Shows the spectral shifts for the nanostructure conjugates generated using a thiol-mediated conjugation protocol, of (i) 50 nm nanostructures prior to conjugation; (ii) 50 nm nanostructures conjugated to CI antibody; (iii) 50 nm nanostructures conjugated to C6 antibodies; (iv) CI -conjugated nanostructures after blocking with BSA; and (v) C6-conjugated nanostructures after blocking with BSA.
• Figure 9 Shows lateral flow strips striped with Protein A (0.5 mg/mL), dipped in a solution containing the conjugated nanostructures generated using the thiol-mediated protocol, or the conjugated nanostructures generated using the thiol-mediated protocol and blocked with BSA.
• Figure 10A Shows the changes in the composite lambdamax for CI and C6 conjugates generated using 50 nm nanostructures and the adsorptive protocol.
• Figure 10B Shows the changes in the composite lambdamax for CI and C6 conjugated generated using 50 nm nanostructures and the thiol-mediated conjugation protocol.
• Figure 11 Shows the effect of the presence of accelerant on the spectral shift for the conjugates prepared by the adsorptive (left panel; 0.25% PEG) and thiol-mediated (right panel; 1% PEG) protocols.
• Figure 12. shows the dose-response curve and kinetics over time in the presence of increasing amounts of antigen (TSH), using covalently linked conjugates in the presence of 0.1% PEG and 0.5% methylcellulose.
• TSH antigen
• Figure 13 Shows reaction curves obtained in the absence (0 ng) or the presence of 0.25 ng of hTSH for different ratios of CI and C6 antibodies in the conjugates (0 parts Cl/40 parts C6, top left panel; 40 parts Cl/0 parts C6, top right panel; 30 parts Cl/10 parts C6, middle left panel; 20 parts Cl/20 parts C6, middle right panel; 10 parts Cl/30 parts C6, bottom panel).
• Figure 14 A Shows peak shift for the conjugates in the presence of increasing amounts of TSH and 0.5% PEG.
• Figure 14B Shows peak shift for the conjugates in the presence of increasing amounts of TSH and 1.0% PEG.
• Figure 15A shows the conjugation of anti-hTSH antibodies CI and C6 to the 70 and 90 nm nanostructures and their reactivates with Protein A lateral flow strips.
• Figure 15B shows that Protein A lines on nitrocellulose reacted as expected before and after blocking with BSA.
• Figure 16 Shows the spectral shift of conjugates comprising about 70 nm diameter nanostructures.
• Figure 17 Shows the spectral shift of conjugates comprising about 90 nm diameter nanostructures.
• Figure 18 Shows detection of TSH measured by the peak shift of 50 nm nanostructures comprising a plurality of protrusions versus nanorods.
• Figure 19 Shows the net peak shift of CHAPS-treated conjugates comprising nanostructures having a plurality of protrusions, conjugated to antibodies at pH 6.0.
• Figure 20 shows an image of a Biolipidure® polymer substrate with a polar charged head group, and a tail that has varying properties from hydrophobic, anionic, cationic, and/or hydrogen bond donating groups.
• the image is from the website of NOF corporation, from which Biolipidure® reagents are commercially available.
• Figure 21 shows the wavelength shift with respect to time of anti-TSH coated nanoparticles that are blocked with a range of Biolipidure® reagents and BSA. Compared to BSA conjugates, blocking with 1002, 1201, 1202, 205 and 206 all enhance the sensitivity of the conjugates in 10 minutes compared to the standard BSA conjugate.
• Figure 22A and 22B show the nonspecific adsorption of the conjugates blocked with Biohpidure® reagents 1002, 1003, 1201, 1202, 205, 206, and BSA ( Figure 22A). Due to the large wavelength shift from 1003, Figure 22B shows the nonspecific adsorption of only 1002, 1201, 1202, 205, 206, and BSA.
• Figure 23 shows the wavelength shift in canine serum of the nanoparticle conjugates with BSA blocking reagents vs 4 of the Biohpidure® blocking reagents that have shown the greatest effect on both improving the sensitivity and reducing the nonspecific wavelength shift in serum.
• Figure 24 shows the improvement of the wavelength shift in response to 1 ng/mL which is diluted 1/20 for a final concentration of 50 pg/mL cTSH antigen in TBS BSA buffer.
• This figure compares the positive response of 80 nm spheres blocked with BSA vs Biohpidure® 1002 and 90 nm nanourchins blocked with BSA vs Biohpidure® 1002. In both cases the Biohpidure® blocked reagent improves the wavelength shift with response to antigen.
• the assay conditions for the results provided in Figure 24 included the following: 50 mM Tris, 150 mM NaCl, 1% BSA, at a pH of 7.7
• Figure 25 provides a schematic of the Hofmeister series salts (Zhang Y, Cremer PS, "Interactions between macromolecules and ions: The Hofmeister series” Curr Opin Chem Biol. 2006 Dec; 10(6):658-63).
• Figure 26 shows the impact of the presence of MgC12 on the levels of non-specific binding in the assay, using nanosphere cTSH conjugates.
• Kilo and Mister are two different normal canine serum samples.
• Figure 27 shows the impact of the presence of MgC12, NaCl, or NaSCN on non-specific binding.
• Figure 28 shows the LSPR peak shift results after 5 minutes from the study testing the presence of MgC12, NaCl, or NaSCN
• Figure 29 shows the effects of the presence of Mg on non-specific binding in the LSPR assay.
• Figure 30 shows the effects of the presence of EDTA on non-specific binding in the LSPR assay.
• the present invention is based, in part, on the discovery that significant amplification in LSPR-based assays can be achieved with anisotropic metallic nanostructure-labeled binding partners.
• the present invention provides analyte detection methods utilizing a plurality of detection conjugates comprising anisotropic metallic nanostructures coupled to biomolecules.
• the metallic nanostructures provided herein are multibranched, anisotropic nanoparticles that comprise a plurality of protrusions on the surface.
• the nanostructures comprising a plurality of protrusions on the surface as provided herein are also at least about 50 nm in diameter.
• the metallic nanostructures provided herein are spherical or non-spherical metallic nanostructures.
• the present invention overcomes problems of current immunoassays, ligand-receptor binding assays, nucleic acid-protein binding assays or other specific binding partner assays that generally require multiple steps and sophisticated equipment to perform such steps.
• the lack of sensitivity and the complexity involved in performing such heterogeneous assays arises from the specific need to separate labeled from unlabeled specific binding partners.
• the present invention overcomes such limitations by performing all steps involved in the assay in a homogenous format wherein the separation of reacted and unreacted assay components is unnecessary as the binding events change LSPR characteristics that are measured in real time by any of the spectroscopic techniques used by those of ordinary skill in spectroscopy.
• one pot assays of the present invention use refractive index sensing, plasmon coupling and related effects to provide amplification of the final LSPR modulated signals.
• the provided methods and metallic nanostructures are capable of improved detection.
• the provided methods and metallic nanostructures are capable of improved detection and minimized non-specific binding (referred to herein as "NSB").
• the present disclosure provides anisotropic nanostructure-antibody conjugates, and methods of making the same, that provide unexpectedly high sensitivity of detection of analytes.
• the present disclosure provides anisotropic nanostructure-antibody conjugates, and methods of making the same, that provide the unexpectedly high sensitivity of detection of analytes while providing unexpectedly low levels of NSB.
• the nanostructures comprise a plurality of protrusions.
• the sensitive detection achieved with such star-shaped nanostructures is unexpected because it was well known in the art that metallic nanoparticles in the shape of a rod are better sensors of refractive index compared to round, spherical, or other nanostructures.
• the superior effects of anisotropic nanostructure with spherical cores and multiple spikes, provided herein are surprising considering that the literature reports suggest better sensitivity with nanorods rather than the star-shaped structures described here.
• the nanostructures are star-shaped or spherical, and the sensitivity and low levels of NSB provided herein is achieved by the conjugation methods provided herein.
• the present invention may be applied to the detection of a variety of antigenic analytes, such as those associated with infectious diseases in both humans and animals, e.g., antigens associated with infectious diseases and antibodies generated in response thereto.
• antigens and antibodies the techniques described herein may also be used for performing assays involving specific binding partners such as ligands and receptors, and transcription factors and their associated DNA binding elements.
• RNA-RNA, RNA-DNA, DNA-DNA or protein-nucleic acid interactions may be detected using appropriate conjugates of anisotropic metallic nanoparticles with specific binding partners.
• the present invention describes the use of metallic nanoparticles in solution (as opposed to being attached to a surface via chemical or physical deposition) to determine the binding of specific binding partners in a qualitative or quantitative manner.
• the changes in the characteristics of light interacting with the regions containing unbound and bound partners attached to metallic nanoparticles can be measured, allowing for both qualitative and quantitative interactions between the specific binding partners to be determined by suitable detectors.
• the present application provides methods of detecting a target analyte in a sample.
• the methods comprise mixing the sample with a plurality of detection conjugates that comprise anisotropic metallic nanostructures coupled to binding partners.
• the nanostructures include a plurality of protrusions, or spikes.
• the nanostructures are at least 50nm in diameter, inclusive of the protrusions.
• the nanostructures are spherical.
• the nanostructures are gold nanostructures.
• the methods comprise a first detection conjugate and a second detection conjugate, wherein the first and second detection conjugates comprise metallic nanostructures coupled to binding partners that are capable of specifically binding to the target analyte if present in the sample to form a complex between the first detection conjugate, the analyte, and the second detection conjugate.
• the conjugates comprise a first binding partner and a second binding partner that each bind to a different epitope on the same target analyte.
• the methods comprise exposing the complex to a light source at a wavelength range within the ultraviolet-visible- infrared spectrum; and measuring an optical signal from the complex, wherein a change in the optical signal indicates the presence of the target analyte in the sample.
• the metallic nanostructure in the first detection conjugate and/or the second detection conjugate is a gold metallic nanostructure.
• the step of mixing occurs in the presence of a polymeric material selected from polyethylene glycol (PEG), polyvinylpyrrolidone, polyallylamine, polyethyleneimine, polylysine, polyacrylic acid, polyvinylalcohol, polyglutamic acid and polyaspartic acid.
• the polymeric material is PEG.
• the step of mixing occurs in the presence of a polysaccharide or other viscosity enhancer.
• the viscosity enhancer selected from trehalose, maltodextrin, sucrose, sorbitol, mannitol, polyvinylpyrrolidone (PVP), or polyvinyl alcohol (PVA).
• the polysaccharide is selected from maltodextrin, trehalose, sucrose, corn syrup, and polyglucose.
• the polysaccharide is maltodextrin or trehalose.
• the step of mixing occurs in the presence of a blocking agent.
• the blocking agent is selected from bovine serum albumin (BSA), casein, gelatin, ovalbumin, and gamma-globulins.
• the blocking agent is BSA.
• the present disclosure provides methods and compositions that include blocking agents that have previously been used in assays such as lateral flow assays, but have not previously been used or contemplated for use in LSPR assays.
• the present disclosure provides methods and compositions for the LSPR assay described herein, wherein one or more Biolipidure® reagent is used as a blocking agent.
• Biolipidure® reagents are polymer agents that exhibit one or more of the following features: enhancement of sensitivity and accuracy of detection; suppression of non-specific adsorption; stabilization of antibodies and enzymes; and elimination of lot-to-lot variations.
• Biolipidure® reagents do not require biohazardous handling and, in some embodiments, are used by preparing a buffer solution with Biolipidure ® (e.g., about 0.1wt%, about 0.25wt%, about 0.5wt%, about 0.75wt%, about lwt%, about 1.25wt%, about 1.5wt%, about 2wt%, about 5wt%, or more), and dissolving the sample to be tested in the buffer.
• the Biolipidure® reagent is used at a concentration of 1 wt%.
• the methods of the present invention can be configured in a sandwich assay format, a direct assay format, an indirect assay format, as well competitive and secondary labelling formats.
• the detection methods are sandwich assays.
• the detection conjugates comprise the anisotropic metallic nanostructures provided herein, coupled to binding partners that are capable of specifically binding to the target analyte if present in the sample.
• the method in a sandwich assay format comprises a first detection conjugate and a second detection conjugate wherein the first and second detection conjugates comprise spherical metallic nanostructures and/or metallic nanostructures having a plurality of protrusions, wherein the nanostructures are coupled to binding partners that are capable of specifically binding to the target analyte if present in the sample to form a complex between the first detection conjugate, the analyte, and the second detection conjugate.
• the metallic nanostructure in the first detection conjugate and/or the second detection conjugate is anisotropic gold metallic nanostructure.
• the complex is exposed to a light source and an optical signal is measured, wherein a change in the optical signal indicates the presence of analyte in the sample.
• the target analyte binds to the binding partners in the detection conjugates to form a complex between the first detection conjugate, the analyte, and the second detection conjugate.
• This complex formation brings the metallic nanostructures in the detection conjugates in close proximity to each other, i.e., plasmon-plasmon coupling.
• the amount of light that is absorbed, scattered, or transmitted by the metallic nanostructures is affected by the proximity of the metallic nanostructures in the complex and thus produces an enhanced shift in the peak absorption wavelength, which indicates the presence of the target analyte in the sample.
• the detection methods are competitive assays.
• the first detection conjugate comprises metallic nanostructures coupled to the target analyte of interest.
• the second detection conjugate is capable of specifically binding to the target analyte.
• the first detection conjugate will bind to the second detection conjugate initially. If a sample containing a target analyte is mixed with these initial complexes, the unlabeled or free target analyte in the sample will compete with the first detection conjugate for binding to the second detection conjugate.
• the change in optical signal in this type of assay will result from the displacement of the metallic nanostmctures in the first detection conjugate from the second detection conjugate, which will proportionately reduce the wavelength shift in the peak absorption wavelength.
• the methods of the invention may utilize a plurality of detection conjugates.
• Detection conjugates comprise spherical metallic nanostmctures or metallic nanostmctures having a plurality of protrusions and coupled to binding partners capable of specifically binding to a target analyte or another detection conjugate depending on the assay configuration.
• the detection conjugates comprise metallic nanostmctures coupled or conjugated to binding partners that are capable of specifically binding a target analyte.
• at least one of the detection conjugates comprises the metallic nanostmctures coupled or conjugated to target analyte s.
• the detection conjugates comprise binding partners that are capable of specifically binding to a target analyte.
• binding partners that are capable of specifically binding to a target analyte.
• specific binding refers to binding to a target molecule with high affinity, e.g., an affinity of at least 10 "6 M.
• the binding partners are haptens and other small molecules, drugs, hormones, biological macromolecules including, but not limited to, antibodies or fragments thereof (e.g., Fv, Fab, (Fab) 2 , single chain, CDR etc.), antigens, receptors, ligands, polynucleotides, aptamers, polypeptides, polysaccharides, lipopolysaccharides, glycopeptides, lipoproteins, or nucleoproteins.
• the binding partners are antibodies.
• the binding partners are antigens.
• the detection conjugates e.g., a first detection conjugate and a second detection conjugate
• a first detection conjugate and a second detection conjugate can both be antibodies that recognize a target analyte, but the epitope to which the first detection conjugate binds the target analyte is separate from and ideally non-overlapping with the epitope to which the second detection conjugate binds the target analyte.
• the first detection conjugate comprises an antibody that recognizes a first epitope of a target analyte and the second detection conjugate comprises a different antibody that recognizes a second epitope of a target analyte.
• the first detection conjugate may comprise a monoclonal antibody that recognizes a first epitope of a target analyte.
• the second detection conjugate may comprise a monoclonal antibody that recognizes a second epitope of a target analyte that is separate from and ideally non-overlapping with the epitope that is recognized by the first detection conjugate.
• the first detection conjugate and/or the second detection conjugate may comprise a polyclonal antibody.
• the first detection conjugate may comprise a polyclonal antibody while the second detection conjugate comprises a monoclonal antibody.
• the first detection conjugate comprises a polyclonal antibody and the second detection conjugate comprises a polyclonal antibody.
• the metallic nanostructures in the detection conjugates can be composed of a noble metal or composite thereof.
• the metallic nanostructures in the detection conjugates may be composed of a transition metal or composite thereof.
• the metallic nanostructures in the detection conjugates may comprise an alkali metal or lanthanide in combination with a noble or transition metal.
• metallic nanostructures in the detection conjugates comprise a metal selected from gold, silver, copper, platinum, palladium, ruthenium, rhodium, osmium, iridium, titanium, chromium, cadmium, zinc, iron, cobalt, nickel, and composites thereof.
• the metallic nanostructures are gold nanostructures.
• the metallic nanostructures are silver nanostructures.
• the metallic nanostructures in the detection conjugates are composite metallic nanostructures.
• “Composite metallic nanostructures” refers to nanostructures that comprise at least two noble metals, transition metals, alkali metals, or lanthanides. The two or more metals may be mixed together, as in an alloy, or the two or more metals may be present in separate portions of the nanostructure. For example, one metal may form the core of the nanostructure, whereas the second metal forms an outer shell or coating of the nanostructure.
• the composite metallic nanostructures comprise at least two metals selected from gold, silver, copper, platinum, palladium, ruthenium, rhodium, osmium, iridium, titanium, chromium, cadmium, zinc, iron, cobalt, and nickel. In other embodiments, the composite metallic nanostructures comprise at least two metals selected from gold, silver, copper, platinum, palladium, cadmium, iron, nickel, and zinc. In one particular embodiment, the composite metallic nanostructures comprise gold and silver. In another embodiment, the composite metallic nanostructures comprise gold and copper. In yet another embodiment, the composite metallic nanostructures comprise silver and copper.
• the composite metallic nanostructures used in the methods of the invention comprise a core of a first metal and a coating of a second metal.
• the composite metallic nanostructures may comprise a silver core and a gold coating.
• the composite metallic nanostructures comprise a copper core and a gold coating.
• the core is silver and the coating is copper.
• each of the composite metallic nanostructures comprises a dielectric core (e.g. silicon dioxide, gold sulfide, titanium dioxide, silica, and polystyrene), a first coating of a first metal, and a second coating of a second metal.
• the core comprising a first metal is dissolved following the coating process with a second metal to create a hollow structure comprised of the second metal.
• a silver core with gold nanoparticles generates a gold shell around the silver core and the silver core is subsequently dissolved or degraded resulting in the formation of a hollow nanogold shell structure.
• the nanostructures disclosed herein include a plurality of protrusions, such as spikes or cone-shaped protrusions.
• the nanostructures provided herein are multibranched nanoparticles.
• the surface of the inner core of the nanostructures is essentially covered by the protrusions.
• the diameters of the nanostructures as recited herein includes the protrusions, i.e., the recited diameters are tip-to-tip of the protrusions covering the nanostructures.
• the average diameter of the nanostructures provided herein having a plurality of protrusions or spikes is from about 50 nm to about 120 nm.
• the average diameter of the nanostructures is inclusive of the protrusions thereon.
• the average diameter is described herein as the tip-to-tip diameter in some embodiments.
• the average diameter is about 50 nm, about 60 nm, about 70 nm, about 80 nm, about 90nm, about 100 nm, about 110 nm, about 120 nm, or more.
• the average diameter is about 70 nm. In other embodiments, the average diameter is about 90 nm.
• the nanostmctures include a mix of average diameters from about 50 nm to about 90 nm.
• the average diameter of the spherical nanostructures provided is from about 50 nm to about 120 nm.
• the average diameter of the spherical nanostructures is about 50 nm, about 60 nm, about 70 nm, about 80 nm, about 90nm, about 100 nm, about 110 nm, about 120 nm, or more.
• the present disclosure provides reaction mixtures comprising the binding partner - nanostructure conjugates disclosed herein.
• the reaction mixtures comprise one or more capping reagent and/or one or more zwitterionic detergent.
• the capping agent is a zwitterionic detergent.
• the reaction mixture comprises CHAPS. The present inventors surprisingly found that the presence of CHAPS, a capping agent and a zwitterionic detergent, allowed the nanostructures provided herein, comprising a plurality of surface protrusions, to be effectively conjugated to binding partners such as antibodies. In addition, the presence of CHAPS allowed for faster centrifugation and shorter time periods for centrifugation.
• the present inventors found that in the presence of CHAPS, centrifugation speeds that would normally cause the anisotropic nanoparticle antibody conjugates to fall apart (e.g., above 15,000g or about 40,000 g) could be used to centrifuge the nanostructures provided herein.
• CHAPS allows for a more efficient generation of conjugates.
• the presence of CHAPS allowed the facile resuspension of the antibody conjugates following centrifugation.
• conjugates comprising hydrophobic antibodies that otherwise cannot be resuspended following centrifugation are readily resuspended in the presence of CHAPS.
• CHAPS detergent helps prevent nonspecific size/shape changes leading to aggregation.
• the reaction mixtures comprise binding partner- nanostructure conjugates wherein the mixture comprises one or more capping agents or zwitterionic detergents selected from sulfobetaine series, a Triton series (x-100) detergent; a Tween series (Tween 20) detergent, a cationic detergent series such as CTAB, and an anionic detergent such as SDS.
• Methods of conjugating molecules to the metallic nanostructures disclosed herein include conjugation chemistries, such as those involving l-Ethyl-3-[3- dimethylaminopropyl]carbodiimide hydrochloride (EDC), sulfo- HS coupling, hydrophobic binding or thioether chemistry.
• the binding partners or target analytes can be coupled to the metallic nanostructures through various chemical functionalities including thiol, amine, dithiol, acrylic phosphoramidite, azide, or alkynes.
• the molecule can be coupled to the metallic nanostructure indirectly through a larger carrier molecule or protein.
• the carrier protein is not capable of specific interaction with the target analyte.
• protein A or protein G or protein A/G may be conjugated or coupled to the nanoparticles.
• the methods for conjugating molecules to the metallic nanostructures comprising mixing a solution comprising the metallic nanostructures with a solution comprising the binding partner to form a binding partner- nanostructure conjugate; blocking the conjugate with BSA; (c) centrifuging the conjugate; and (d) resuspending the conjugates in a diluent comprising buffer such as PBS, a blocking agent such as BSA and CHAPS.
• the binding partner is an antibody.
• the antibody is an antibody containing hydrophobic regions.
• the metallic nanostructure is adjusted to basic pH prior to titration of the antibody into the nanostructure.
• the nanostructure pH is adjusted to pH of about 8, about 8.5, about 8.8, or about 9.2.
• the pH of the solution comprising the nanostructure can be adjusted to a neutral or acidic pH (e.g., about 5.5, about 6, about 6.5, or about 7) and successfully form conjugates capable of sensitive antigen detection.
• the neutral or acidic pH resulted in conjugates which were difficult to resuspend in standard conjugate diluents comprising BSA and phosphate buffer. Surprisingly such insoluble conjugates were rapidly dissolved in buffers containing CHAPS.
• the metal or metals employed in a first detection conjugate can be the same as the metal or metals from which the metallic nanostructures in the second detection conjugate are fabricated.
• the first detection conjugate comprises gold nanostructures and the second detection conjugate comprise gold nanostructures.
• the metal employed in the first detection conjugate is different from the metal or metals used to create the metallic nanostructures in the second detection conjugate.
• the reaction environment may be adjusted with appropriate buffers, ionic strength, and other accelerants.
• the reaction environment comprises polyethylene glycol (PEG), which, as described herein, can enhance the strength of the LSPR signal and the rate at which the signal develops.
• PEG polyethylene glycol
• Other similar polymeric materials may also be used, including, but not limited to, polyvinylpyrrolidone, polyallylamine, polyethyleneimine, polylysine, polyacrylic acid, polyvinylalcohol, and polyaspartic acid.
• the present invention also provides analyte detection devices for utilizing the methods described herein to detect a target analyte in a sample.
• Suitable analyte detection devices may include, but are not limited to, a spectrophotometric cuvette, an analytical rotor, a microwell plate, or a flow chamber.
• the tip of an optical fiber or a transparent gel may also be employed to carry out the detection methods disclosed herein.
• all components of the analyte detection devices described herein are contained within a centrifugal rotor or disc.
• a rotor or disc may contain one or more reaction chambers in which the plurality of detection conjugates is located.
• the detection conjugates are present in the form of lyophilized compositions, such as lyophilized beads or pellets.
• the analyte detection device comprises a rotor or disc having one or more reaction chambers, wherein each reaction chamber comprises a plurality of detection conjugates (e.g., a first detection conjugate and a second detection conjugate), wherein the detection conjugates are first and the second specific binding partners coupled to metallic nanoparticles.
• Such a device provides a one-step analyte detection assay whereby a test sample is contacted with the rotor or disc, and application of a centrifugal force to the rotor or disc delivers the test sample to the reaction chambers where the sample mixes with the first detection conjugate and the second detection conjugate.
• the detection conjugates can be selected such that a different analyte can be detected in each reaction chamber.
• These rotor-format detection devices can be configured in the sandwich assay format, the direct competitive format, or both if the rotors comprise multiple reaction chambers.
• direct competitive assays or sandwich assays may be performed in a centrifugal rotor, such as a rotor described in US Patent Nos. 5,061,381, 5, 122,284, 5, 186,844, 5,304,348, 5,457,053, and 5,693,233.
• the present disclosure provides multiplex assays in which discs or rotors capable of multiplex analysis allow for separate detection via, for example, multiple cuvettes.
• the nanoparticle conjugates of the two pairing monoclonal antibodies or a polyclonal antibody mixture that binds to more than one epitope are added as lyophilized beads.
• the solution phase LSPR assay works both with monoclonal and polyclonal antibodies.
• the present disclosure provides antibody pairs that allow highly sensitive detection in an LSPR assay.
• the antibody pair is anti-TSH antibody clones CI and C6, which each bind to a different epitope of TSH.
• the antibody pair is anti-TSH antibody close CI and 5409.
• the best signal to noise ratio is obtained with the gold conjugates prepared from anti-TSH close 5405 and 5409.
• kits comprising the analyte detection devices of the invention as disclosed herein.
• the kit comprises a plurality of detection conjugates (e.g., a first detection conjugate and a second detection conjugate), wherein the detection conjugates are specific binding partners linked to the metallic nanostructures provided herein.
• one or more of the detection conjugates may be lyophilized, for example, in the form of a pellet or bead. In one embodiment, all of the detection conjugates are lyophilized.
• the kit may include one or more additional reagents. In some embodiments, one or more of the additional reagents is provided in lyophilized form.
• the kit may comprise a blocking agent, a sugar, a polymeric accelerant material, sodium chloride, and/or combinations thereof.
• a "blocking agent” is an agent that prevents the association of proteins present in the sample with the detectable agent and/or analyte. Blocking agents are typically proteins themselves and may include, but are not limited to, bovine serum albumin (BSA), casein, gelatin, ovalbumin, gamma-globulins, and IgG from non-immunized animals.
• BSA bovine serum albumin
• the sugar is a polysaccharide.
• the polysaccharide is selected from maltodextrin, corn syrup, and polyglucose.
• the polysaccharide is maltodextrin.
• the sugar is trehalose.
• the reagent kit may comprise maltodextrin and trehalose.
• the polymeric accelerant material is PEG.
• the kits of the invention may also include instructions for using the device to detect an analyte in a test sample, devices or tools for collecting biological samples, and/or extraction buffers for obtaining samples from solid materials, such as soil, food, and biological tissues.
• a test sample can be any type of liquid sample, including biological samples or extracts prepared from environmental or food samples.
• the test sample is a biological sample.
• Biological samples include, but are not limited to, whole blood, plasma, serum, saliva, urine, pleural effusion, sweat, bile, cerebrospinal fluid, fecal material, vaginal fluids, sperm, ocular lens fluid, mucous, synovial fluid, peritoneal fluid, amniotic fluid, biopsy tissues, saliva, and cellular lysates.
• the biological sample can be obtained from a human subject or animal subject suspected of having a disease condition, such as cancer, infectious diseases (e.g., viral-, bacterial-, parasitic- or fungal-infections), cardiovascular disease, metabolic disease, autoimmune disease etc.
• a disease condition such as cancer, infectious diseases (e.g., viral-, bacterial-, parasitic- or fungal-infections), cardiovascular disease, metabolic disease, autoimmune disease etc.
• infectious diseases e.g., viral-, bacterial-, parasitic- or fungal-infections
• cardiovascular disease e.g., bacterial-, parasitic- or fungal-infections
• metabolic disease e.g., autoimmune disease etc.
• the test sample is mixed with a first detection conjugate and the mixture is subsequently brought into contact with the second detection conjugate.
• the sample, the first detection conjugate, and the second detection conjugate are brought into contact at the same time. For instance, contact of the sample with both reagents simultaneously may occur in the rotor-format detection devices described herein.
• the present application relates, in some embodiments, to the use of metallic nanostructures conjugated to binding partners, wherein the nanostructures have a plurality of protrusions, such as spikes or cone-shaped protrusions, and wherein the nanostructures have an average diameter of about 50 nm or more.
• the present inventors have surprisingly found that the sensitivity of the solution-based assay is significantly enhanced with protrusion-laden nanostructures compared to the use of nanorods (which have a smooth rod- shaped surface), even though nanorods would have been expected to provide superior results because they are known to be the better sensors of refractive index changes.
• the present inventors surprisingly found that in the solution-based assays disclosed herein, the metallic nanostructure conjugates comprising nanostructures having a plurality of protrusions exhibited robust antigen detection whereas nanorod-conjugates were not capable of robust antigen detection.
• the present inventors have further found that the larger nanostructures comprising protrusions exhibit better sensitivity of detection relative to smaller nanostructures having the same protrusion features.
• the sensitivity of detection increases when the average diameter of the nanostructures used in the assay is increased from about 50 nm to about 70 nm. In further embodiments, the sensitivity of detection increases even more when the average diameter of the nanostructures used in the assay is increased from about 70 nm to about 90 nm.
• the solution comprises a polysaccharide at a final concentration of about 2% to about 20% wt/vol. In another embodiment, the solution comprises a polysaccharide at a final concentration of about 4% to about 15% wt/vol. In yet another embodiment, the solution comprises a polysaccharide at a final concentration of about 5% to about 10% wt/vol. In an exemplary embodiment, the solution comprises a polysaccharide at a final concentration of about 5%, 6%, 7%, 8%, 9%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, 50%, 55%, 60% or more, inclusive of all values therebetween.
• trehalose may be used to prevent sedimentation of detection conjugates in analytical rotors.
• the trehalose concentration is about 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, 50%, 55%, 60% or more, inclusive of all values therebetween
• the sensitivity of the assay may be improved when a polysaccharide is added to the solution as compared to an assay performed in a solution comprising an alternative sugar, e.g., sucrose, trehalose, maltodextrin, sorbitol, mannitol, or ficoll.
• the polysaccharide is maltodextrin.
• the polysaccharide is trehalose.
• the polysaccharide is dextran.
• the solution comprises a blocking agent at a final concentration of about 0.1%) to about 20% wt/vol. In another embodiment, the solution comprises a blocking agent at a final concentration of about 0.5% to about 10% wt/vol. In yet another embodiment, the solution comprises a blocking agent at a final concentration of about 1% to about 5% wt/vol. In an exemplary embodiment, the solution comprises a blocking agent at a final concentration of about 1%), 2%), 3%), 4%, or 5%, inclusive of all values therebetween. In various embodiments described herein, the sensitivity of the assay may be improved when a blocking agent is added to the solution as compared to an assay performed in the absence of a blocking agent. In some embodiments, the blocking agent is selected from bovine serum albumin, casein, gelatin, ovalbumin, and gamma-globulins. In an exemplary embodiment, the blocking agent is bovine serum albumin (BSA).
• BSA bovine serum albumin
• the solution comprises one or more of maltodextrin, trehalose, PEG, a blocking agent (e.g. BSA), and/or sodium chloride.
• one or more of the solution components e.g., maltodextrin
• a liquid e.g., water, saline solution, or a liquid biological sample.
• one or more of the solution components may be provided in a spectrophotometric cuvette or a reaction chamber of an analytical rotor as a bead that is suspended into the solution following the addition of a liquid.
• the LSPR signal may be substantially increased by mixing the first and second detection conjugates with the analyte in the presence of a polymeric accelerant material selected from polyethylene glycol, polyvinylpyrrolidone, polyallylamine, polyethyleneimine, polylysine, polyacrylic acid, polyvinylalcohol, and polyaspartic acid.
• a polymeric accelerant material selected from polyethylene glycol, polyvinylpyrrolidone, polyallylamine, polyethyleneimine, polylysine, polyacrylic acid, polyvinylalcohol, and polyaspartic acid.
• the polymeric material is polyethylene glycol (PEG).
• the reaction mixture comprises a polymeric material, e.g., PEG, at a final concentration of about 0.1 mg/mL to about 200 mg/mL.
• the reaction mixture comprises a polymeric material, e.g., PEG, at a final concentration of about 0.2 mg/mL to about 100 mg/mL. In yet another embodiment, the reaction mixture comprises a polymeric material, e.g., PEG, at a final concentration of about 0.5 mg/mL to about 10 mg/mL. In yet another embodiment, the reaction mixture comprises a polymeric material, e.g., PEG, at a final concentration of about 2 mg/mL to about 8 mg/mL. In an exemplary embodiment, the reaction mixture comprises a polymeric material, e.g., PEG, at a final concentration of about 2, 3, 4, 5, 6, 7, or 8 mg/mL, inclusive of all values therebetween.
• PEG of different molecular weight may be used, e.g., a smaller quantity of higher molecular weight PEG can be used for a substantial effect.
• PEG concentrations required for assay enhancement vary with the molecular weight of the polymer.
• the detection methods of the invention may be used to determine qualitative or quantitative amounts of a target analyte. Such methods are particularly useful for determining the approximate amount of a target analyte in a sample, which can be used inter alia to diagnose certain medical conditions or evaluate the efficacy of a drug therapy.
• the quantity of a target analyte can be determined by establishing a standard curve for the particular analyte by measuring changes in optical signals from the metallic nanoparticles as described herein for samples with a known quantity of target analyte; determining the optical signal change for a test sample; and comparing the optical signal change for the test sample to the values obtained for the standard curve.
• determining the quantity of a complex between a first reagent and a second reagent comprises comparing the absorbance ratio and/or reaction rate from a test sample to the absorbance ratio and/or reaction rate from one sample with a known quantity of complex, thereby determining the quantity of the complex in the test sample.
• the quantitative values obtained from test samples may be compared to pre-determined threshold values, wherein said pre-determined threshold values are indicative of either an abnormal or normal level of the target analyte.
• the detection methods of the present invention provide a highly sensitive technique for detecting minute quantities of a target analyte in a sample.
• amplification of surface plasmon resonance-based signals can be achieved with gold nanostructure conjugates such that nanogram quantities of target analyte can be detected in a sample.
• the presence of nanogram quantities of a target analyte is detected.
• plasmon resonance-based signals from detection conjugates comprising gold nanoparticles can be amplified using composite metallic nanostructure detection conjugates. Use of gold-coated silver nanostructures conjugated to an analyte-specific antibody may enable the detection of pictogram quantities of the target analyte.
• the presence of picogram quantities of the target analyte is detected.
• the presence of femtogram quantities of the target analyte is detected. Greater sensitivities may be obtained by altering the composition and/or shape of the composite metallic nanostructures.
• light sources for applying electromagnetic energy suitable for use in the methods of the invention can include any source that may apply a wavelength range within the ultraviolet-visible spectrum or ultraviolet-visible-infrared spectrum, including arc lamps and lasers.
• the light source may be equipped with a monochromator so that specific wavelengths of light may be applied.
• the optical properties of the metallic nanostructures depend on their size, shape, and composition.
• solid gold nanoparticles have an absorption peak wavelength (Xmax) from about 515 nm to about 560 nm depending on particle size.
• Gold spherical nanoparticles having a 30 nm diameter maximally absorb at about 520 nm with Xmax shifting to longer wavelengths as particle diameter increases.
• Silver and copper particles have a max in the ultraviolet/blue or red region (e.g., from about 350 nm to about 500 nm) with increasing particle diameter causing a shift in max to longer wavelengths.
• Metallic nanorods have a transverse Xmaxi and a longitudinal Xmax2.
• Alloys of different metals typically exhibit absorption peaks in an intermediate range between the absorption peaks of the comprising metals.
• nanostructures comprising a 50/50 alloy of gold and silver exhibit a max of about 480 nm with increasing amounts of gold causing a shift in the absorption peak to longer wavelengths.
• the sensitivity of the LSPR signals to changes in the local medium refractive index can be modified by changing the shape or geometry of the nanostructures. For instance, nonspherical particles (e.g. nanoprisms, nanorods, nanoshells, etc.) have increased LSPR sensitivities to changes in refractive index as compared to spheres.
• the optical properties e.g. absorption/scattering at particular wavelengths
• the interaction between the incident light and the metallic nanostructures can be monitored as reflected light or transmitted light.
• the amount of the incident light that is absorbed or scattered can be measured as an absorption spectrum in a reflection mode or the absorption spectrum in a transmission mode.
• the optical signal measured from the metallic nanostructures can be an optical reflection, an absorbance spectrum, a scattering spectrum, and/or an emission spectrum.
• the plasmon coupling between the metallic nanostructures in the detection conjugates resulting from complex formation between the binding partners and target analyte produces a change in the localized surface plasmon resonance spectrum of the metallic nanostructures.
• changes can include an increased optical extinction, an increased optical reflection, and/or increased scattering and/or emission signal.
• the change in optical signal indicative of the presence of the target analyte in the sample includes a shift, increase or decrease in optical scattering or a combination of these features.
• the change in optical signal indicative of the presence of the target analyte in the sample is a spectral peak wavelength shift.
• the change in optical signal indicative of the presence of the target analyte in the sample is the wavelength shift at a position other than the peak.
• the change in optical signal indicative of the presence of the target analyte in the sample may be the midpoint spectral wavelength shift, the spectral wavelength shift at the wavelength' s base, or the total spectral wavelength shift such as difference spectrum.
• the wavelength shift in the optical spectral peak may be a red shift (e.g., a shift to a longer wavelength) within a 200 nm to 1200 nm spectral window.
• the wavelength shift in the optical spectral peak may be a blue shift (e.g., a shift to a shorter wavelength) within a 200 nm to 1200 nm spectral window.
• the changes in optical signals can be measured at a particular time point following a set reaction period. Additionally or alternatively, changes in the optical signal over the reaction period (e.g. rate determinations) may be measured. Both types of measurements can be used for either qualitative or quantitative analysis of a target analyte.
• spectrophotometric or photometric instruments are suitable for use in the disclosed methods.
• Some non-limiting examples include plate readers, Cobas Fara analyzers, and Piccolo xpress® and Vetscan analyzers (Abaxis, Inc., Union City, CA), optic fiber readers (e.g., LightPathTM S4 (LamdaGen, Menlo Park, CA)), SPR instruments (e.g., Biacore instruments available from GE Healthcare), centrifugal analyzers from Olympus, Hitachi etc.
• the present invention also includes an assay complex comprising (i) a first detection conjugate that comprises the metallic nanostructures provided herein having a plurality of protrusions, coupled to a binding partner, (ii) a target analyte, and (iii) a second detection conjugate that comprises a metallic nanostructure according to the present disclosure, coupled to a binding partner, wherein the binding partner in the first detection conjugate is bound to a first epitope on the target analyte and the binding partner in the second detection conjugate is bound to a second epitope on the target analyte, thereby forming a complex comprising the first detection conjugate, target analyte, and the second detection conjugate.
• the assay complex is contained within a cuvette adapted for use with a centrifugal rotor. In other embodiments, the assay complex is contained within a reaction chamber in a centrifugal rotor or disc.
• target analyte can be detected using the methods, devices, and assay complexes of the present invention, particularly those that are significant in the diagnoses of diseases.
• a target analyte can include, but is not limited to, a protein, enzyme, antigen, antibody, peptide, nucleic acid (RNA, DNA, mRNA, miRNA), hormone, glycoprotein, polysaccharide, toxin, virus, virus particle, drug molecule, hapten, or chemical.
• the target analyte is a marker or antigen associated with an infectious disease in humans and/or animals.
• the target analyte is a marker or antigen associated with a particular physiological state or pathological condition.
• the target analyte is a pathogenic antigen or antibody to a pathogenic antigen.
• the pathogenic antigen can be a viral antigen (e.g., feline leukemia virus, canine parvovirus, foot and mouth virus, influenza virus, hepatitis a, b, c virus, HIV virus, human papilloma virus, Epstein Barr virus, rabies virus, etc.), a bacterial antigen (e.g., Ehrlichia, Borrelia, Anaplasma, Salmonella, Bacillus, Rickettsia, etc.), a fungal antigen, or parasitic antigen (e.g., canine heartworm, Giardia lamblia, plasmodium falciparum, African trypanosomiasis, Trypanosoma brucei, etc.).
• a viral antigen e.g., feline leukemia virus, canine parvovirus, foot and mouth virus, influenza virus, hepatitis a,
• the bacterial antigen may be from Ehrlichia canis, Ehrlichia chaffeensis, Ehrlichia ewingii, Borrelia burgdorferi, Anaplasma platys, Anaplasma phagocytophilum, Salmonella enterica, Bacillus anthracis, and Rickettsia rickettsii.
• the target analyte is a disease-related antigen or antibody to a disease-related antigen.
• Disease-related antigens include, but are not limited to, cancer-related antigens or markers (e.g., PSA, AFP, CA125, CA15-3, CA19-9, CEA, NY-ESO- 1, MUC1, GM3, GD2, ERBB2, etc.), cardiovascular disease-related antigens or markers (e.g., troponin, C-reactive protein, brain natriuretic peptide, CKMB, fatty acid binding protein, etc.,), metabolic-related antigens or markers (e.g., thyroid stimulating hormone, thyroxine, leptin, insulin), or autoimmune disease-related antigens or markers (e.g., auto-antibodies).
• cancer-related antigens or markers e.g., PSA, AFP, CA125, CA15-3, CA19-9, CEA, NY-ESO- 1, MUC1, GM3, GD2, ERBB2, etc.
• cardiovascular disease-related antigens or markers e.g., troponin, C-
• the target analyte is an inflammatory antigen or marker (e.g., C-reactive protein, MRP14, MRP8, 25F9, etc.). In other embodiments, the target analyte is a pregnancy-related antigen or marker (e.g., a fetal antigen, human chorionic gonadotropin). [0106] In some embodiments, the present disclosure provides methods for synthesizing the nanostructure provided herein.
• an inflammatory antigen or marker e.g., C-reactive protein, MRP14, MRP8, 25F9, etc.
• the target analyte is a pregnancy-related antigen or marker (e.g., a fetal antigen, human chorionic gonadotropin).
• silver/gold nanoparticles are synthesized in a single vessel by adding predetermined quantities of the following reagents in succession and with thorough mixing: (1) a surfactant (e.g., ionic [anionic, cationic or zwitterionic], or non- ionic) or capping agent such as 3-((3-Cholamidopropyl) dimethylammino)-l-propanesulfonate (CHAPS), SDS, Tween, Triton, or any of the sulfobetaine detergents, (2) gold chloride, (3) water, (4) silver nitrate, (5) trisodium citrate and finally (6) ascorbic acid is added to initiate the formation of nanoparticles.
• a surfactant e.g., ionic [anionic, cationic or zwitterionic], or non- ionic
• capping agent such as 3-((3-Cholamidopropyl) dimethylammino)-l-propanesulfonate (
• the nanoparticles are synthesized in a single vessel by adding predetermined quantities of the following, in the following order: (1) a surfactant or capping agent such CHAPS, SDS, Tween, Triton, CTAB, or any of the sulfobetaine detergents, (2) gold chloride, (3) silver nitrate, (4) trisodium citrate, (5) water, and (6) a reductant.
• the reductant is made up of CHAPS, ascorbic acid, trisodium citrate, and water.
• the reductant is made up of about 200 mg CHAPS, about 4g ascorbic acid, about 1 17.6 mg trisodum citrate, and about 15.68 g water.
• about 1 mL of aqueous 1% (wt/wt) CHAPS is mixed sequentially with about 0.25 mL of 0.1M gold chloride, about 0.5 mL of 0.02M silver nitrate, about 0.05 mL of 1M trisodium citrate, about 6.2 mL of water, and about 2 mL of the reductant.
• concentrations of various active ingredients such as metallic salts, capping agents, reductants and pH of the solution results in different particle types (e.g., nanospheres, nanostars or nanorods) and different composition of the nanoparticles.
• nanostars are formed by mixing, in order, water, cetyltrimethylammonium bromide (CTAB), gold chloride, ascorbic acid, and pre-formed gold nanosphere seeds.
• CTAB cetyltrimethylammonium bromide
• gold nanosphere seeds about 0.825 mL of water, about 0.1 mL of 20% CTAB, about 0.025 mL of 0.1 M gold chloride, about 0.05mL of 1M ascorbic acid, and about 0.05 mL of gold nanosphere seeds are mixed in that order.
• the age of the seeds and the ratio of seeds to the metallic ions influence the geometry and thus the optical spectra of nanoparticles.
• Gold only nanostars are fabricated by reducing gold chloride using the reductant that is made up of about 200 mg CHAPS, about 4g ascorbic acid, about 117.6 mg trisodum citrate, and about 15.68 g water.
• the size of nanostars formed is dictated by the gold chloride concentration.
• the gold nanostars prepared by this method can be purified by centrifugation and stored in water at 2-8°C. [0108]
• the formation of nanomaterials using the methods provided herein is essentially complete within minutes but may be allowed to reach equilibrium overnight. The synthesis of nanoparticles can be monitored by spectroscopy and confirmed by scanning or transmission electron microscopy.
• the size and thus the optical properties can be changed by altering the concentration of the surfactant or capping agent, ascorbic acid, trisodium citrate, gold chloride and/or silver nitrate.
• the size of nanostars synthesized increases with increasing silver content up to a certain point and then it decreases. These changes are reflected in the LSPR peak of the synthesized nanostars as the peak red-shifts at increasing silver/gold ratio but then starts to blue shift at molar ratios of Gold: Silver: :5 :2.
• the final concentrations of the chosen detergent in the reaction mixture can be varied from 0.05-5% with the smaller particles predominating at higher concentrations of the detergent.
• Increasing the concentrations of ascorbic acid produces smaller nanostars with the final concentration of ascorbic acid varying from 0.05 to 0.2M.
• increasing concentration of trisodium citrate from 10 mM to 100 mM decreases the nanostar sizes.
• gold-silver nanoalloys may be synthesized under alkaline reduction conditions by mixing CTAB (e.g., CTAB dissolved in alcohol) with gold chloride and silver nitrate.
• CTAB e.g., CTAB dissolved in alcohol
• nanoalloy formation may be induced by mixing, in order, water, CTAB, gold chloride (0.5 mM to 5 mM), silver nitrate (20% to 80% of gold), ascorbic acid (10 mM to 200 mM) or a reductant containing ascorbic acid, trisodium citrate and CHAPS, and NaOH (50% to 200% of ascorbic acid).
• nanoalloys are formed by mixing about 0.825 ml of water, about 0.1 ml of 20% CTAB prepared in isopropanol, about 0.025 ml of 0.1M gold chloride, about 0.005-0.025ml of 0.1M silver nitrate, about 0.05 ml of 1M ascorbic acid, and about 0.05 ml of 1M NaOH.
• the concentrations of CTAB can be varied from 0.05M to 0.2M with lower concentrations favoring higher content of nanostars synthesized. Acidic pH favors formation of nanorods and higher aspect ratios are obtained at decreasing pH.
• CI and C6 conjugates were recovered by centrifugation, washed once with the conjugate diluent and re-centrifuged. The sediments containing conjugates were easily dissolved in a conjugate storage solution containing PBS/BS A/CHAPS. Dilutions of the final conjugates were made in water and compared. The original unconjugated nanostructures had peak at 573.8 nm which red-shifted to 585-586 nm in the blocked conjugates. The shift is shown in Figure 5. The final conjugate solutions may be stored at 2-8C until use.
• nanostructures having a plurality of protrusions and an average diameter of 50 nm were adjusted to pH 8.8 with 0.1M borate.
• CI or C6 antibodies (about 33 picomoles per OD nanostructure) were titrated in and mixed well for 15 minutes. 2mg BSA per ml was added and mixed for a further 15 minutes.
• Nanostructure/Cl or /C6 mixtures were centrifuged for 15,000 g for 10 minutes; supernatant was removed; and the conjugates were resuspended in conjugate diluent CG-1P, comprising PBS/BSA and CHAPS.
• CHAPS was particularly important to the resuspension of C6 antibodies, which are hydrophobic. Moreover, the CHAPS detergent helped prevent nonspecific size/shape changes leading to aggregation.
• Figure 6 shows the spectral shifts, for conjugates generated using the adsorptive protocol, of (i) 50 nm nanostructures prior to conjugation; (ii) 50 nm nanostructures conjugated to CI antibody; (iii) 50 nm nanostructures conjugated to C6 antibodies; (iv) CI -conjugated nanostructures after blocking with BSA; and (v) C6-conjugated nanostructures after blocking with BSA.
• the study shows that the antibody binding caused 4-5 nm red-shift, and an additional shift of 1 nm was induced upon blocking of conjugates with BSA.
• nanostructures having a plurality of protrusions and an average diameter of 50 nm kmax at 575 nm - 1.0 OD/mL were adjusted to pH 8.8 with 0.1M borate.
• TCEP-reduced CI or C6 antibodies (about 33 picomoles per OD nanostructure) were titrated in and mixed well for 15 minutes. 2mg BSA per ml was added and mixed for a further 15 minutes.
• Nanostructure/Cl or /C6 mixtures were centrifuged for 15,000 g for 10 minutes; supernatant was removed; and the conjugates were resuspended in conjugate diluent CG-1P, comprising PBS/BSA and CHAPS.
• CHAPS was particularly important to the resuspension of C6 antibodies, which are hydrophobic. Moreover, the CHAPS detergent helped prevent nonspecific size/shape changes leading to aggregation.
• Figure 8 shows the spectral shifts, for conjugates generated using the thiol-mediated conjugation protocol, of (i) 50 nm nanostructures prior to conjugation; (ii) 50 nm nanostructures conjugated to CI antibody; (iii) 50 nm nanostructures conjugated to C6 antibodies; (iv) Cl- conjugated nanostructures after blocking with BSA; and (v) C6-conjugated nanostructures after blocking with BSA.
• the study shows that the antibody binding caused 4-5 nm red-shift, and an additional shift of 1 nm was induced upon blocking of conjugates with BSA.
• Figure 10A shows the changes in the composite max for CI and C6 conjugates generated using 50 nm nanostructures and the adsorptive protocol.
• Figure 10B shows the changes in the composite max for CI and C6 conjugated generated using 50 nm nanostructures and the thiol-mediated conjugation protocol.
• Figure 12 shows the dose-response curve and kinetics over time in the presence of increasing amounts of antigen (TSH), using covalently linked conjugates in the presence of 0.1% PEG and 0.5% methylcellulose.
• Figure 12 shows the peak shift dose response of covalently linked conjugates of anti-TSH CI and C6 in the presence of 0.1% polyethylene glycol and 0.5% methylcellulose.
• Example 5 Larger nanostructures having a plurality of spikes and average diameters of 70 or 90 nm
• FIG. 15A shows the conjugation of anti-hTSH antibodies CI and C6 to the 70 and 90 nm nanostructures and their reactivities with Protein A lateral flow strips.
• Figure 15B shows that Protein A lines on nitrocellulose reacted as expected before and after blocking with BSA.
• the unconjugated 70 and 90 nm nanostructures showed Xmax of 609.5 and 641.9, respectively.
• the attachment of C I and C6 followed by blocking with BSA caused up to 8 nm shift in Xmax.
• the table below shows the quantified data from Figure 15 A.
• Example 6 Activity of nanostructures having a plurality of protrusions versus nanorods in the solution-based assay
• Nanorods (45.5 ⁇ 6.3 nm in length and 17.4 ⁇ 1.2 nm in width) were obtained from Nanocomposix and conjugated to antibody clones 1 and 6 via an adsorptive conjugation protocol. 50 nm nanostructures comprising a plurality of protrusions were also conjugated to antibody clone 1 and 6 using passive adsorption at pH9.2 in borate buffer as described above. The results of the study are provided in Figure 18. The ability of the nanorod conjugates to detect TSH was tested in a buffer comprising PBS, BSA and 1% PEG 20000 with or without the addition of 10 ng of TSH.
• Figure 18 shows that there was no net change in Xmax, which was calculated by subtracting values obtained with TSH from those without TSH; Xmax changes were recorded using Nicoya Lifesciences' OpenSPRTM. Nanostructures having a plurality of protrusions were tested similarly but the amount of TSH was 0.5 ng as the rates were too fast at TSH concentrations of 10 ng/ml. Strikingly, the nanostructures comprising a plurality of protrusions exhibited robust TSH detection as measured by peak shift analysis, whereas the nanorods failed to detect TSH. This result was unexpected at least because nanorods are believed to be excellent sensors of refractive index changes. However, in the present solution-based assay, nanostructures having a plurality of protrusions, and not nanorods, exhibit superior effects.
• Example 7 Low-pH conjugation protocol yields conjugates exhibiting sensitive detection
• Anti-TSH antibody clones CI and C6 were conjugated to gold nanostars prepared by a single vessel seed-free method.
• Clones 1 and 6 were separately added to the nanostar solutions to obtain 5 ⁇ g of the antibody per OD of the nanostar solution.
• the conjugates were blocked with 2 mg BSA per ml of the conjugate.
• the conjugates were then separated from reactants by centrifugation at 25000 g for 15 min. The centrifugation may be repeated if the pellets are loose by adding 10 mM phosphate buffered BSA (1%).
• the final sediment is dissolved in the following CHAPS containing buffer: PBS(lx), BSA (1%) and CHAPS (2%). Dissolution is aided by sonication for up to 30 seconds.
• Example 8 Simultaneous reduction in nonspecific adsorbance of serum proteins and increase of immunoassay sensitivity
• Biolipidure® reagents are synthetic polymeric reagents that contain a phosphorylcholine (PC) polar group, and a polymeric tail that contains hydrophobic, anionic, cationic, and/or hydrogen bond donating groups, Figure 20. These reagents are also known as 2- methacryloyloxyethyl phosphorylcholine polymers (MPC) that have been incorporated into polymeric biomaterials due to their properties of resisting nonspecific protein adsorption, cell adhesion, and blood coagulation. Some features of these reagents include enhancement of sensitivity and accuracy, suppression of non-specific adsorption, stabilization of antibodies and enzymes, reduction of lot-to-lot variation without the hassle of biohazardous handling.
• PC phosphorylcholine
• MPC 2- methacryloyloxyethyl phosphorylcholine polymers
• the Biolipidure® reagents are added to a final working solution in order to achieve the desired results of the product.
• the Biolipidure® reagents can be applied by coating microplates, coating magnetic beads, and by adding to the antibodies that are present in solution.
• Biolipidure® reagents can be used by preparing a buffer solution with lwt% of Biolipidure® reagent; dissolving the sample (for example, mucosa) in the buffer, and loading the diluted sample on the sample pad of the immunochromatograph.
• the Biolipidure® reagents can both reduce nonspecific adsorption of serum proteins, and enhance the sensitivity of the assay. Briefly, gold nanospheres were coated with mouse IgG for 15 min, followed by one of the Biolipidure® blocking agents, 205, 206, 1002, 1003, 1201, 1202, or BSA for 15 min. The antibody-gold conjugates were washed 3x and suspended in conjugate diluent for storage prior to testing.
• the wavelength shift of BSA blocked IgG conjugates over the time course of 10 minutes in response to the addition of canine serum was around 3.5 nm.
• the Biolipidure® conjugate 1202 showed a similar wavelength shift as the BSA blocked conjugates.
• the conjugates blocked with 205, 206, 1002, and 1201 all showed a decrease in wavelength shift in the presence of canine serum. [0140] Due to the varying properties of Biolipidure® reagents, they have different responses to canine serum, and enhancing the sensitivity of a sandwich immunoassay.
• Biolipidure® reagents 205, 206, 1002, and 1201 all show the capability to both reduce the wavelength shift with canine serum, and improve the LSPR shift in response to antigen in this homogeneous sandwich immunoassay.
• Biolipidure® reagent 1202 was able to improve the response to antigen, while the wavelength shift in response to the addition of canine serum to the sample was equivalent to that of the BSA conjugates.
• nanourchin i.e., anisotropic nanoparticles that comprise a plurality of protrusions on the surface
• Biolipidure® reagent 1002, 2x for 1 ng/mL of antigen diluted 20 fold to 50 pg/mL of canine antigen, Figure 24.
• These conjugates are also much more sensitive than the spherical gold conjugates blocked with Biolipidure® 1002.
• the results of the study provided a surprising method for increasing sensitivity while decreasing non-specific binding in the assay.
• Changing the blocking agent during the gold nanoparticle-antibody passive conjugation procedure from BSA to some Biolipidure® reagents resulted in a significant increase in wavelength shift to antigen in buffer conditions, and there was a decrease in the wavelength shift in response to the addition of serum to the conjugates, indicating a likely decrease in nonspecific adsorption from serum components.
• PBS-BSA 100 m gCL2 0.552 ; 0.285
• PBS-BSA 50 mM gCL2 0.448 ; 0.875 0.334 0.322
• PBS-BSA REP2 1.035 : 3.070

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